Among the
many ways to find fragments, one of the relatively
inexpensive newcomers is weak affinity chromatography, or
WAC (see also
here).
The technique works by immobilizing a target protein onto a column and flowing
fragments over it; molecules that bind to the target will elute more slowly
than those that don’t. WAC has a number of potential benefits, but as with any
technique the question is how well it really works. In a
paper published a few
months ago in
Analytical Chemistry,
Sten Ohlson at Linnaeus
University and
collaborators at Vernalis compared WAC with more established methods.
The protein they chose, HSP90, is sort of the fruitfly of
FBLD: just about every technique has been tested on it. It’s also an oncology
target with which Vernalis has
many years of experience. The researchers chose
111 fragments from the Vernalis library and screened these using WAC. They also
screened most of the fragments using surface plasmon resonance (
SPR),
fluorescence polarization (FP),
thermal shift, and NMR (using three techniques:
STD, waterLOGSY, and relaxation filtered spectra; only fragments that confirmed
in all three NMR assays were considered hits).
The
top 27 hits from WAC were also investigated with isothermal titration
calorimetry (
ITC), and 32 hits were soaked into crystals for X-ray
crystallography.
The results were quite encouraging, with good agreement
between the different methods:
NMR performed the best, though this could be due in part to
the fact that three separate NMR techniques were used. Thermal shift performed
the worst, with both false positives as well as false negatives, but even here
the agreement was always greater than 50%. It is also important to note that
assay conditions varied from technique to technique (for example, the pH ranged
from 6.5 to 7.5), which could account for many of the discrepancies.
These results are in sharp contrast to some other
comparisons of fragment finding methods (such as
here and
here), which showed
little or no correlation between hits. Why the difference? One possibility is
that the folks at Vernalis have worked out all the kinks in their assays and
are very adept at separating the true hits from the chaff. Of course, it
probably doesn’t hurt that they were working with a well-behaved and
extensively characterized target.
The main focus of the paper is WAC, which performed
admirably. Compounds could be screened in pools of up to 16 fragments when
mass-spectrometry was used as a detection method, and less than 2 milligrams of
HSP90 was used to prepare all three of the WAC columns made. One worry with
immobilizing your protein is long term stability, but the columns seemed to be
stable for at least 6 months through multiple runs.
Of course, no technique is perfect, and one area where WAC
gets whacked is in determining dissociation constants. The correlation between
KD values measured by SPR and ITC was excellent (R2 =
0.91) but much worse for WAC versus ITC (R2 = 0.38) and nonexistent
for WAC versus SPR (R2 = 0.016), though some of this could possibly
be explained by differences in buffer conditions.
Overall it looks like WAC is a great way to find fragments,
though you may want to use other methods to actually quantify binding. This
paper provides a detailed guide for using WAC, as well as good descriptions of
other fragment-finding methods.